首页> 美国卫生研究院文献>The Journal of Clinical Investigation >Direct method for detecting small quantities of hepatitis B virus DNA in serum and plasma using the polymerase chain reaction.
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Direct method for detecting small quantities of hepatitis B virus DNA in serum and plasma using the polymerase chain reaction.

机译:使用聚合酶链反应直接检测血清和血浆中少量乙肝病毒DNA的方法。

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摘要

Serum components inhibit DNA polymerase, thereby obviating direct detection of serum viral DNA sequences by the polymerase chain reaction (PCR). This has necessitated extraction of nucleic acid from sera before performing PCR and has resulted in loss of sensitivity. By adsorbing virus to a solid surface (microcentrifuge tubes or antibody coated microparticles) followed by proteinase K digestion, as little as three viruses per 200 microliters serum may be directly detected by PCR without nucleic acid extraction. The sensitivity is dependent on the surface area of the adsorptive surface and is increased by having antibodies on the adsorptive surface. The nucleic acid sequence of the amplified DNA fragments may be directly determined by the dideoxy method. Of 24 plasma samples from HBsAg+ volunteer blood donors, HBV DNA was detected in 7 by dot blot assay, 7 by liquid hybridization, and 9 by PCR. PCR detected DNA in every sample that was positive by another assay. Analysis of serial samples of two patients with acute self-limited hepatitis B found detectable HBsAg and pre-S2 antigenemia before HBV DNA by the PCR method. These results suggest that surface antigenemia may precede viremia during acute hepatitis.
机译:血清成分抑制DNA聚合酶,从而避免了通过聚合酶链反应(PCR)直接检测血清病毒DNA序列。这需要在进行PCR之前从血清中提取核酸,并导致灵敏度降低。通过将病毒吸附到固体表面(微量离心管或抗体包被的微粒),然后进行蛋白酶K消化,可以直接通过PCR检测每200微升血清中少至三种病毒,而无需提取核酸。灵敏度取决于吸附表面的表面积,并通过在吸附表面上具有抗体来提高灵敏度。扩增的DNA片段的核酸序列可以通过双脱氧法直接确定。在来自HBsAg +自愿献血者的24份血浆样品中,通过斑点印迹法检测到HBV DNA,通过液体杂交检测到7份,通过PCR检测到9份。 PCR检测到每个样品中通过另一种检测呈阳性的DNA。通过PCR方法分析了两名急性自限性乙型肝炎患者的系列样本,发现在HBV DNA之前可检测到HBsAg和S2前抗原血症。这些结果表明在急性肝炎期间表面抗原血症可能先于病毒血症。

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